The present invention provides a use of a lipid composition for the preparation of a nutritional, pharmaceutical or nutraceutical composition or a functional food, for the prevention and treatment of gastrointestinal diseases and disorders, and for promoting intestinal development, maturation, adaptation and differentiation.
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1. A method for treating in a subject short bowel syndrome, inflammatory bowel diseases and necrotizing enterocolitis, and for promoting in a subject intestinal development, maturation, adaptation and differentiation, said method comprising:
administering to the subject a therapeutically effective amount of a lipid composition which comprises at least one synthetic triglyceride of the following formula I:
##STR00007##
wherein R1, R2 and R3 may be identical or different and are each independently selected from H or an acyl group;
wherein said acyl group is selected from a group consisting of saturated, mono-unsaturated and poly-unsaturated fatty acid residues with the proviso that R2 is a palmitic acid residue; and
wherein the total palmitic acid residue content is from about 15% to about 55% of the total fatty acid residues in the lipid composition; and wherein at least 30% of the total palmitic acid residues are bonded in the composition at the sn-2 position of the triglyceride backbone.
2. The method of
4. The method of
5. The method of
6. The method of
7. The method of
8. The method of
0-10% C8:0 fatty acids out of the total fatty acids;
0-10% C10:0 fatty acids out of the total fatty acids;
0-22% C12:0 fatty acids out of the total fatty acids;
0-15% C14:0 fatty acids out of the total fatty acids;
15-55% C16:0 fatty acids out of the total fatty acids;
wherein at least 30% at sn-2 position;
1-7% C18:0 fatty acids out of the total fatty acids;
20-75% C18:1 fatty acids out of the total fatty acids;
2-40% C18:2 fatty acids out of the total fatty acids;
0-8% C18:3 fatty acids out of the total fatty acids; and other fatty acids are present in levels of less than 8% of the total fatty acids.
9. The method of 1, wherein said lipid composition is prepared from a natural, synthetic or semi-synthetic source.
10. The method of 9, wherein the production of said lipid composition involved an enzymatic catalysis.
11. The method of 1, wherein said composition is a nutritional composition, a pharmaceutical composition, a nutraceutical composition or a functional food.
12. The method of
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This application is a continuation of U.S. Ser. No. 12/682,311, filed Apr. 9, 2010, which is a §371 national stage of PCT International Application No. PCT/IL2008/001311, filed Oct. 2, 2008, which claims priority to U.S. Provisional Application No. 60/960,664, filed Oct. 9, 2007, the entire contents of each of which are hereby incorporated by reference in their entirety into this application.
This invention relates to the field of gastrointestinal diseases and disorders and intestinal development and maturation.
Adequate neonatal nutrition is essential for appropriate growth and to avoid complications associated with nutritional deficiencies. Neonatal nutritional requirements vary with metabolic states, degree of prematurity and diseases affecting the gastrointestinal, pulmonary, and cardiac systems.
Infants may suffer from several digestive system disorders that may vary from light discomforts to sever life threatening diseases.
The rising incidence of preterm births, coupled with improved survival as a result of highly evolving technologies, has resulted in an increased need to develop innovative and cost-effective treatment modalities for preterm infants during the neonatal period and in later life. Pre-term babies do not achieve the intestinal maturity normally accreted during the third trimester of pregnancy, and are often born with immature gastrointestinal tract, and gastrointestinal diseases and disorders.
US2003/0072865 describes an infant formula comprising a lipid component in which palmitic acid residues make up more than 10% of total fatty acid residues present in the triglycerides resulting in reduced constipation, abdominal discomfort, and gastrointestinal problems.
Postnatal phases lead to maturation of intestinal epithelial cells occur in the early life of an animal: morphogenesis and cytodifferentiation prepare the epithelium for digestion and absorption of colostrums and milk components; thickening of the mucosa occurs due to the growth of villi and crypts.
Epithelial structure and function of the gastrointestinal tract in neonates changes abruptly before weaning to adapt to a change in feeding from milk to solid food. Although intestinal maturation in the neonate has been the subject of intensive studies, the factors triggering the major biochemical and morphologic changes during maturation are still poorly understood. Newborn infants have a very immature cell lining in the intestines. The junctions between enterocytes are not tight, and the brush border and mucus layers are not fully developed. Due to the less tight mucosal barrier, the infant is at greater risk of contracting infections and developing allergies. Thus, intestinal maturation and differentiation of the gut barrier to protect against environmental aggression is desired
During life, intestinal epithelial cells have to fulfill different roles, including classical digestive and absorptive functions, maintenance of a barrier against noxious antigens and bacteria, and secretion of water and electrolytes to keep a proper viscosity of the luminal contents and flush out oxious components.
Intestinal development, maturation, adaptation and differentiation are highly important in the course of a subject's life.
The present invention provides a use of a lipid composition comprising at least one triglyceride of the following formula I:
##STR00001##
wherein R1, R2 and R3 may be identical or different and are each independently selected from H or an acyl group, wherein said acyl group is selected from a group consisting of saturated, mono-unsaturated and poly-unsaturated fatty acid residues, and wherein the total palmitic acid residue content is from about 15% to about 55% of the total fatty acid residues in the composition, for the preparation of a nutritional, pharmaceutical or nutraceutical composition or a functional food, for the prevention and treatment of gastrointestinal diseases and disorders, and for promoting intestinal development, maturation, adaptation and differentiation.
The subject invention further envisages a method of treating a subject having, or having an increased risk of, gastrointestinal disease or disorder, and of promoting intestinal development, maturation, adaptation and differentiation comprising administering to the subject a lipid composition comprising at least one triglyceride of the following formula I:
##STR00002##
wherein R1, R2 and R3 may be identical or different and are each independently selected from 1 or an acyl group, wherein said acyl group is selected from a group consisting of saturated, mono-unsaturated and poly-unsaturated fatty acid residues and wherein the total palmitic acid residue content is from about 15% to about 55% of the total fatty acid residues in the composition.
In order to understand the invention and to see how it may be carried out in practice, embodiments will now be described, by way of non-limiting example only, with reference to the accompanying drawings in which:
§p<0.05 Diet A or Diet B vs Diet C
†p<0.05 Diet A vs Diet B
§p<0.05 Diet A or Diet B vs Diet C
†p<0.05 Diet A vs Diet B
§p<0.05 Diet A or Diet B vs Diet C
†p<0.05 Diet A vs Diet B
The present invention provides a use of a lipid composition comprising at least one triglyceride of the following formula I:
##STR00003##
wherein R1, R2 and R3 may be identical or different and are each independently selected from H or an acyl group, wherein said acyl group is selected from a group consisting of saturated, mono-unsaturated and poly-unsaturated fatty acid residues, and wherein the total palmitic acid residue content is from about 15% to about 55% of the total fatty acid residues in the composition, for the preparation of a nutritional, pharmaceutical or nutraceutical composition or a functional food, for the prevention and treatment of gastrointestinal diseases and disorders, and for promoting intestinal development, maturation, adaptation and differentiation.
The lipid composition used in the invention typically comprises a mixture of said triglycerides of formula I. Such a mixture comprises two or more triglycerides of formula I.
The present invention further envisages a method of treating a subject having, or having an increased risk of, gastrointestinal disease or disorder, and of promoting intestinal development, maturation, adaptation and differentiation comprising administering to the subject a lipid composition comprising at least one triglyceride of the following formula I:
##STR00004##
wherein R1, R2 and R3 may be identical or different and are each independently selected from H or an acyl group, wherein said acyl group is selected from a group consisting of saturated, mono-unsaturated and poly-unsaturated fatty acid residues and wherein the total palmitic acid residue content is from about 15% to about 55% of the total fatty acid residues in the composition.
The present invention further envisages a method of preventing a gastrointestinal disease or disorder in a subject comprising administering to the subject a lipid composition comprising at least one triglyceride of the following formula I:
##STR00005##
wherein R1, R2 and R3 may be identical or different and are each independently selected from H or an acyl group, wherein said acyl group is selected from a group consisting of saturated, mono-unsaturated and poly-unsaturated fatty acid residues and wherein the total palmitic acid residue content is from about 15% to about 55% of the total fatty acid residues in the composition.
Compositions of the subject invention are intended for treating or preventing gastrointestinal diseases and disorders in a subject, and for promoting intestinal development, maturation, adaptation and differentiation.
The “subject” as used herein should be understood to encompass any mammal, including, but not limited to, humans, household animals (e.g. cat, dog), and farm animals (e.g. cow, goat, ship). Said subject may be in any stage of development or maturity in its life cycle. The subject can be, but is not limited to, a newborn, a preterm and term infant, a toddler, a child, an adolescent, an adult or a geriatric subject.
An infant as used herein can be any infant, such as, but not limited to, a newborn, a preterm and term infant, small premature infants, which are susceptible to immature gastrointestinal tract, infants with very low birth weight (VLBW) or extreme low birth weight (ELBW), particularly those with increased risk of necrotizing enterocolitis and others.
A composition as used herein can be, but is not limited to, a nutritional composition (such as infant formula), a nutraceutical composition (such as a dietary supplement), a functional food, a medical food, or a pharmaceutical composition.
In one embodiment, a lipid composition for use in the invention is prepared from a natural, synthetic or semi-synthetic source. In a further specific embodiment, said natural source is any one of plant, animal or microorganism source. In yet a further embodiment, the production of said lipid composition involves an enzymatic catalysis.
A nutritional composition as used herein can be any nutritional composition including, but not limited to, human milk fat substitute, infant formula, dairy product, ice-cream, biscuit, soy product, bakery, pastry and bread, sauce, soup, prepared food, frozen food, condiment, confectionary, oils and fat, margarine, spread, filling, cereal, instant product, infant food, toddler food, bar, snack, candy and chocolate product.
A functional food as used herein can be any functional food, including, but not limited to, dairy product, ice-cream, biscuit, soy product, bakery, pastry and bread, sauce, soup, prepared food, frozen food, condiment, confectionary, oils and fat, margarine, spread, filling, cereal, instant product, drinks and shake, infant food, bar, snack, candy and chocolate product.
A nutraceutical composition as used herein can be any nutraceutical, which can be any substance that may be considered a food or part of a food and provides medical or health benefits, including the prevention and treatment of disease. Such nutraceutical compositions include, but are not limited to, a food additive, a food supplement, a dietary supplement, genetically engineered foods such as for example vegetables, herbal products, and processed foods such as cereals, soups and beverages and stimulant functional food, medical food and pharmafood.
In an embodiment of the invention, the pharmaceutical or nutraceutical compositions are in a dosage delivery form.
Suitable routes of administration for the compositions of the subject invention are oral, buccal and sublingual administration or administration via a feeding tube. In a specific embodiment, the compounds are administered orally.
The exact dose and regimen of administration of the composition will necessarily be dependent upon the therapeutic effect to be achieved (e.g. treatment of gastrointestinal disease) and may vary with the particular formula, the route of administration, and the age and condition of the individual subject to whom the composition is to be administered.
The present invention thus also provides pharmaceutical compositions for use in the invention in admixture with pharmaceutically acceptable auxiliaries, and optionally other therapeutic agents. The auxiliaries must be “acceptable” in the sense of being compatible with the other ingredients of the composition and not deleterious to the recipients thereof.
In one embodiment, the pharmaceutical composition further comprises at least one pharmaceutically active agent.
The compositions may be prepared by any method well known in the art of pharmacy. Such methods include the step of bringing in association the ingredients with any auxiliary agent. The auxiliary agent(s), also named accessory ingredient(s), include those conventional in the art, such as carriers, fillers, binders, diluents, disintegrants, lubricants, colorants, flavouring agents, anti-oxidants, and wetting agents.
Pharmaceutical compositions suitable for oral administration may be presented as discrete dosage units such as pills, tablets, dragées or capsules, or as a powder or granules, or as a solution or suspension.
The compositions may be presented in unit-dose or multi-dose containers, for example sealed vials and ampoules, and may be stored in a freeze-dried (lyophilised) condition requiring only the addition of sterile liquid carrier, for example water, prior to use.
The invention further provides a commercial package for preparing a composition for use in the invention such as an edible fat source or food article in accordance with the invention comprising (a) a fat source which upon enteral administration to a subject prevents or treats digestive system disorders, and/or promotes intestinal development, maturation, adaptation and differentiation; (b) optionally at least one of edible physiologically acceptable protein, carbohydrate, vitamin, mineral, amino acid, nucleotide and active or non-active additive; (c) optionally at least one edible physiologically acceptable carrier or diluent for carrying the constituent/s defined in (a) and (b); (d) means and receptacles for admixing the constituents defined in (a), (b) and/or (c); and (e) instructions for use such as, but not limited to terms of storage, instructions for preparation of the fat source or food article for administration, required dilutions, dosages, frequency of administration and the like.
A commercial package in accordance with the invention may also contain a fat source of the invention in a ready-to-use form, together with instructions for use. Dosages are usually determined according to age, weight, sex and condition of the subject, in accordance with good medical practice known to the attending physician and other medical personnel.
Gastrointestinal disease or disorder as used herein should be understood to encompass gastroesophageal reflux (GER), Gastroesophageal reflux disease (GERD), necrotizing enterocolitis (NEC), Hyperbillirubinemia, Inflammatory bowel diseases (such as but not limited to Crohn's disease and Ulcerative colitis), short bowel syndrome, intestinal ections or incisions, intestinal re-anastomosis, ulcer, surgical interventions for example for treating intestinal adhesions, and intestinal obstruction.
The term “intestine” as used herein should be understood to encompass a segment of the alimentary canal extending from the stomach to the anus. In humans and other mammals, the intestine consists of two segments, the small intestine (in humans further subdivided into the duodenum, jejunum and ileum) and the large intestine (in humans further subdivided into the cecum and colon). Other mammals may have a further complexed intestine.
Promoting intestinal development as used herein should be understood to encompass promoting a process or part of a process of enhancing, increasing, growing, supporting or advancing the formation of a specialized mature epithelium. Promoting intestinal maturation as used herein should be understood to encompass promoting a process or part of a process of enhancing, increasing, growing, supporting or advancing the differentiation processes of enterocyte and intestinal segments.
Both intestinal (segment) development and maturation may be measured by intestinal mucosal parameters such as, but not limited to bowel circumference, bowel weight and mucosal weight and by histological changes such as but not limited to villus height and crypt depth.
Promoting intestinal adaptation as used herein should be understood to encompass any physiological change by which the absorptive capacity of the small intestine is enhanced, increased, grown, supported or advanced including, but not limited to, enlargement or lengthening of the villi found in the lining, increase in the diameter of the small intestine and slow down in peristalsis or movement of food through the small intestine.
Promoting intestinal differentiation as used herein should be understood to encompass a process by which a pre-differentiated cell becomes a specialized cell type. For example, in case of intestinal differentiation, pluripotent stem cells, localized near the base of the crypt, are subsequently differentiated into one of the four primary cell types: absorptive enterocytes, goblet cells, Paneth cells, and enteroendocrine cells.
GER (Gastroesophageal reflux) is a disorder wherein the liquid gastric contents are squirted backwards. Instead of squirting down into the intestines, they squirt up into the esophagus. In infants the major cause of GER is immaturity of lower esophageal sphincter. When the reflux damages the esophagus it is called GERD.
GERD (Gastroesophageal reflux disease) is a disorder with chronic symptoms or mucosal damage produced by the abnormal reflux in the esophagus. This is commonly due to transient or permanent changes in the barrier between the esophagus and the stomach. GERD is more evident in babies having pre mature or a not fully developed gastro intestinal tract.
Hyperbillirubinemia is common and in most cases a benign problem. The color usually results from the accumulation in skin of unconjugated, non-polar, lipid-soluble billirubin pigment. The toxic effect of elevated levels of unconjugated billirubin in serum is increased by several factors, such as free fatty acids, that reduce the retention of billirubin in the circulation.
NEC is a gastrointestinal disease that mostly affects premature infants; it involves infection and inflammation that causes destruction of the bowel (intestine) or part of the bowel. NEC is the most common and serious gastrointestinal disorder among hospitalized preterm infants.
Studies have shown that the risk of NEC is increased as the infant is born earlier and that the risk of breast fed infants is lower than infants that are formula-fed.
NEC typically occurs after milk feeding has begun. Premature infants have immature bowels, which are sensitive to changes in blood flow and prone to infection.
The exact cause of NEC is unknown, but several theories exist. It is thought that the intestinal tissues of premature infants are weakened by too little oxygen or blood flow, and when feedings are started, the added stress of food moving through the intestine allows bacteria that are normally found in the intestine to invade and damage the wall of the intestinal tissues.
The infant is unable to continue feedings and starts to appear ill if bacteria continue to spread through the wall of the intestines and sometimes into the bloodstream. Because the infant's body systems are immature, even with quick treatment for NEC there may be serious complications.
Other factors seem to increase the risk of developing NEC. Some experts believe that the makeup of infant formula, the rate of delivery of the formula, or the immaturity of the mucous membranes in the intestines can cause NEC. inflammatory bowel disease (IBD) is a group of inflammatory conditions of the large intestine and small intestine. The major types of IBD are Crohn's disease and ulcerative colitis. Ulcerative colitis is an inflammatory disease of the large intestine. In ulcerative colitis, the inner lining—or mucosa—of the intestine becomes inflamed (meaning the lining of the intestinal wall reddens and swells) and develops ulcers meaning an open, painful wound. Inflammatory bowel disease (BED) may cause symptoms such as, but not limited to, bloody stools, occult blood in the stool, body weight loss, bloody diarrhea, reduced physical activity, severe anemia, shortened colonic length, and perianal injury. Crohn's disease differs from ulcerative colitis in the areas of the bowel it involves—it most commonly affects the last part of the small intestine (called the terminal ileum) and parts of the large intestine. However, Crohn's disease isn't limited to these areas and can attack any part of the digestive tract. Crohn's disease causes inflammation that extends much deeper into the layers of the intestinal wall than ulcerative colitis does. Crohn's disease generally tends to involve the entire bowel wall, whereas ulcerative colitis affects only the lining of the bowel.
Short bowel syndrome (SBS) is a malabsorption disorder caused by the surgical removal of the small intestine, or rarely due to the complete dysfunction of a large segment of bowel. Most cases are acquired, although some children are born with a congenital short bowel. SBS usually does not develop unless a person has lost more than two thirds of their small intestine.
Surgical intervention as used herein should be understood to encompass an intervention for e.g. diagnosis and/or treatment of injury, deformity, or disease. Such intervention may involve an operation or procedure in the gastrointestinal tract, such as, but not limited to, an intestinal section or incision and intestinal reanastomosis. Such an intestinal section or incision may be a cut or a wound made by cutting the intestine with a sharp instrument, such as one used during surgery.
Intestinal reanastomosis is a connection between two vessels in the body. Surgical anastomosis involves the deliberate joining of two vessels or hollow parts of an organ; for example, when part of the intestine has been removed and the remaining free ends are brought together and stitched.
Intestinal adhesions are bands of fibrous tissue that can connect the loops of the intestines to each other, or the intestines to other abdominal organs, or the intestines to the abdominal wall. These bands can pull sections of the intestines out of place and may block passage of food. Adhesions are a major cause of intestinal obstruction. Adhesions may be present at birth (congenital) or may form after abdominal surgery or inflammation.
Intestinal obstruction refers to the partial or complete mechanical or nonmechanical blockage of the small or large intestine. Infants under one year of age are most likely to have intestinal obstruction caused by meconium ileus, volvulus, and intussusception. Meconium ileus, which is the inability to pass the first fecal excretion after birth (meconium), is a disorder of newborns. It may also occur in very low birth weight (VLBW) infants. In meconium ileus, the abnormal meconium must be removed with an enema or through surgery. Volvulus is twisting of either the small or large bowel, that may cut off the blood supply to the bowel, leading to tissue death (gangrene). In intussusception, the bowel telescopes into itself like a radio antenna folding up. It is most common in children between the ages of three and nine months, although it also occurs in older children. Almost twice as many boys suffer intussusception as girls.
A fat source is used in the preparation of a composition (such as an infant formula) for use in the subject invention. Such composition, for example an infant formula, may further comprise other components such as, but not limited to a protein source, a carbohydrate source, minerals, vitamins, nucleotides, amino acids and optionally at least one of a carrier, diluent, additive or excipient, all of which are edible.
A fat blend as used herein for the preparation of a composition for use in the invention, such as an infant formula, can be, but is not limited to, any fat source, such as those described in WO05/036987, which include fat concentrates (also named fat bases). The fat blend used in the present invention can be any dietary ingredient comprising an edible fat source. In a particular embodiment, fat blends are those which are based on synthetic triglycerides (which can be produced both chemically and enzymatically) which mimic the triglyceride composition of human breast milk fat. In one embodiment, such fat base (and fat blend) contains a high level of palmitic acid at the sn-2 position of the triglycerides of formula I (e.g., at least 30%), and a high level of unsaturated fatty acids at sn-1 and sn-3 positions of the triglyceride of formula I (e.g. at least 50% of the total fatty acid at sn-1 and sn-3 positions). A non-limiting example is a blend named InFat® (Enzymotec Ltd., Migdal HaEmeq, Israel).
##STR00006##
Since fat blends are prepared by blending fat base with other oils, the fatty acid composition of the fat blends results from the fatty acid composition of both the fat base and the other oils mixed with the fat base.
Infant formula used in the subject invention can be a substitute human milk fat composition comprising a fat blend consisting of at least 25% of a fat base with up to 75% of at least one vegetable oil.
Non-limiting examples of vegetable oil used in the preparation of blends used in the invention are soy, palm tree, canola, coconut, palm kernel, sunflower, corn and rapeseed oil, as well as other vegetable oils and fats and mixtures thereof.
As used herein, the term “lipid” related to fats and fatlike compounds, which are essentially insoluble in water and which include, but are not limited to, triglycerides, sterols, fatty acids, and so forth.
As used herein, the term “acyl group” relates to an organic radical denoted —C(═O)R, wherein R is selected from saturated, mono-unsaturated and polyunsaturated C4-C2 aliphatic residue of the fatty acid residue.
As used herein, the term “fatty acid” relates to a carboxylic acid with a long unbranched aliphatic tail (chain), which is either saturated or unsaturated having one unsaturated bond (mono-unsaturated fatty acids) or two or more unsaturated bonds (poly-unsaturated fatty acids).
Non-limiting examples of saturated fatty acids which may be used in this invention include: Butyric acid (Butanoic acid, C4:0), Caproicacid (Hexanoic acid, C6:0), Caprylic acid (Octanoic acid, C8:0), Capric acid (Decanoic acid, C10:0), Laurie acid (Dodecanoic acid, C12:0), Myristic acid (Tetradecanoic acid, C14:0), Palmitic acid (Hexadecanoic acid, C16:0), Stearic acid (Octadecanoic acid, C18:0), Arachidicaicd (Eicosanoic acid, C20:0), Behenic acid (Docosanoic acid C22:0).
Non-limiting examples of unsaturated fatty acids which may be used in this invention include: Myristoleic acid (ω-5, C14:1), Palmitoleic acid (ω-7, C16:1), Oleic acid (ω-9, C18:1), Linoleic acid (ω-6, C18:2), Alpha-linolenic acid (ω-3, C18:3), Arachidonic acid (ω-6, C20:4), Eicosapentaenoic acid (ω-3, C20:5), Erucic acid (ω-9, C22:1) and Docosahexaenoic acid (ω-3, C22:6).
In one embodiment of the invention, R2 is a saturated fatty acid residue. In a further embodiment, the saturated fatty residue is selected from C14-C18 saturated fatty acid residues. In yet a further embodiment, the saturated fatty acid is a palmitic acid residue.
In one embodiment, the total palmitic acid residue content is from about 15% to about 40% of the total fatty acid residues in the composition. In another embodiment, the total palmitic acid residue content is from about 15% to about 33% of the total fatty acid residues in the composition.
In another embodiment of the invention, R1 and R3 are both H.
In one embodiment, at least 13% of the total fatty acids at the sn-2 position of the triglyceride backbone are palmitic acid residues. In another embodiment, at least 15% of the total fatty acids at the sn-2 position of the triglyceride backbone are palmitic acid residues. In yet another embodiment, at least 18% of the total fatty acids at the sn-2 position of the triglyceride backbone are palmitic acid residues. In yet another embodiment, at least 22% of the total fatty acids at the sn-2 position of the triglyceride backbone are palmitic acid residues.
In one embodiment, at least 30% of the total palmitic acid residues in the composition are bonded at the sn-2 position of the triglyceride backbone. In another embodiment, at least 33% of the total palmitic acid residues are bonded at the sn-2 position of the triglyceride backbone. In yet another embodiment, at least 38% of the total palmitic acid residues are bonded at the sn-2 position of the triglyceride backbone. In yet another embodiment, at least 40% of the total palmitic acid residues are bonded at the sn-2 position of the triglyceride backbone.
In a further embodiment of the invention, R1 and R3 are unsaturated fatty acid residues.
In one embodiment, at least 50% of the total fatty acid residues at the sn-1 and sn-3 positions of the triglyceride backbone are unsaturated. In a further embodiment, at least 70% of the total fatty acid residues at the sn-1 and sn-3 positions of the triglyceride backbone are unsaturated. In one embodiment, said unsaturated fatty acid residue is selected from the group consisting of oleic acid, linoleic acid, linolenic acid and gadoleic acid. In one specific embodiment, at least 35% of the unsaturated fatty acid residues at the sn-1 and sn-3 positions are oleic acid residues. In a further specific embodiment, at least 40% of the unsaturated fatty acid residues at the sn-1 and sn-3 positions are oleic acid residues.
In one specific embodiment, at least 4% of said unsaturated fatty acid residues at the sn-1 and sn-3 positions are linoleic acid residues. In a further specific embodiment, at least 6% of said unsaturated fatty acid residues at the sn-1 and sn-3 positions are linoleic acid residues.
In a first embodiment, said lipid composition consists of:
In a second embodiment, said lipid composition consists of:
All possible combinations of said first and said second embodiments are also envisaged.
For example:
It is to be understood that the compounds provided herein may contain chiral centers. Such chiral centers may be of either the (R) or (S) configuration, or may be any mixture thereof. Thus, the compounds provided herein may be enantiomerically pure, or be stereoisomeric or diastereomeric mixtures such as racemic or non-racemic mixtures.
The invention is further described in the following examples, which are not in any way intended to limit the scope of the inventions as claimed.
Compositions
Table 1 details the contents of several fat bases enriched with a high content of palmitic acid at the sn-2 position (hereinafter “fat bases”). Table 2 details the contents of several fat sources (hereinafter “fat blends”) comprising either fat base 1, 7, 8, 9, 10 or 11 for use in the subject invention.
The fat base may represent about 30% up to about 83% of the fat blends suitable for use in a formula for use in the invention.
The preparation of these fat sources is essentially as described in WO05/036987.
TABLE 1
fat base 1
fat base 2
fat base 3
fat base 4
fat base 5
fat base 6
fat base 7
fat base 8
fat base 9
fat base 10
fat base 11
C12:0
C14:0
C16:0
32
29.4
29.6
32.6
32.2
30.6
29
29
30
33
30
C16:0 at sn-2
67.2
59.7
61.3
66.1
66
62.9
53.9
55.6
59
52.9
55.8
of total fatty
acids at sn-2
Ratio (%) of
70.0
67.7
69.0
67.6
68.3
68.5
62
64
64
53.5
62
sn-2 palmitic
acid of total
palmitic acid
C18:0
4
4.4
4.4
4
4.1
3.8
2.6
2.6
3
3
3
C18:1
53.1
55.9
55.5
53.1
53.4
55
55.5
56
56.1
52
56.1
C18:2
8
7.8
8.2
8
7.9
8.3
9
9
8.5
10
8.5
All numbers represent % (w/w), except the ratio which is defined as %. C16:0 represents the total palmitic acid content. C16:0 at the sn-2 represents the % palmitic acid at sn-2 of total sn-2 positioned fatty acids. The ratio means the % of sn-2 palmitic acid of total palmitic acid {(% of sn-2 palmitic of total sn-2 positioned fatty acids)/3)/(% total palmitic acid)} × 100.
TABLE 2
Prepara-
Prepara-
Prepara-
Prepara-
Prepara-
Prepara-
Prepara-
Prepara-
Prepara-
Prepara-
tion A
tion B
tion C
tion D
tion E
tion F
tion G
tion H
tion I
tion J
Fat
Fat
Fat
Fat
Fat
Fat
Fat
Fat
Fat
Fat
blend 1
blend 2
blend 3
blend 4
blend 5
blend 6
blend 7
blend 8
blend 9
blend 10
Fatty acid
C12:0
11.1
7.2
7.8
6.5
4.4
8.1
8.7
13.4
10.1
10
C14:0
4.5
3.1
3.3
2.8
2.1
2.9
3.5
5.3
3.7
4.2
C16:0
22.8
25.4
26.9
25.1
27.7
21.6
21
15
22.1
17
C16:0 at sn-2 of
33.4
42.9
48.9
50.8
56.9
31.3
31.8
25
28.7
16
total fatty acids at
sn-2
Ratio (%) of sn-
48.7
56.3
60.7
67.4
68.5
48.3
50.5
55
43.3
31.5
2 palmitic acid of
total palmitic
acid
C18:0
2.3
3.0
3.1
3.5
4.0
2.6
2.6
2.9
2.7
3.2
C18:1
38.4
40.8
41.6
47.9
46.6
42.7
44.4
39.7
43.9
41.7
C18:2
13.5
15.6
12.8
8.6
11.7
18
16.4
15.3
13.6
18.2
C18:3
1.7
0.6
1.4
1.8
1.5
2
1.4
2.1
% Fat base 1 in
30
50
63
73
83
fat blend
% Fat base 7 in
60
fat blend
% Fat base 8 in
60
fat blend
% Fat base 9 in
36
fat blend
% Fat base 10 in
52
fat blend
% Fat base 11 in
25
fat blend
Vegetable Oil
Palm kernel Oil
18
Coconut oil
23
15
16
13.5
9.3
17
28
21
21
Palm oil
21
15
9
14
Sunflower
5
7.7
11
14
Corn oil
10
10
12
11
safflower
3
5
Rapeseed
16
5
13.5
4
6
20
16
11
Soybean
18
17
Total
100
100
100
100
100
100
100
100
100
100
C16:0 represents the total palmitic acid content. C16:0 at the sn-2 represents the % palmitic acid at sn-2 of total sn-2 positioned fatty acids. The ratio means the % of sn-2 palmitic acid of total palmitic acid (% of sn-2 palmitic of total sn-2 positioned fatty acids)/3)/(% total palmitic acid)} × 100. All numbers represent % (w/w), except the ratio which is defined as %.
Infant Formula
An infant formula comprising a fat base and additional oils and fats (i.e. fat blends) that mimic the human breast milk fat composition were prepared as follows:
The fat fraction was produced by blending of fat base with other oils. Oil was mixed together with other infant formula components (proteins, carbohydrates, minerals, vitamins and others). The slurry was passed through a pressure homogenizer to get a stable emulsion. Homogenized product was then dried in a spray drier to obtain final product. Other additives may be added to the dry powder to obtain final formulation.
The fat fraction produced by the blending of fat base with other oils and fats as described above was further blended with other nutrients such as proteins, minerals, vitamins and carbohydrates to yield a food product supplying an infant with the major nutrients also found in human milk. The nutrients and fats were homogenized using pressure homogenization and spray dried to yield a homogenous powder. The powder was further re-dispersed in water (approx. 9 g powder per 60 ml water) to yield a ready-to-feed formula. The fat content of the ready feed was approx. 3.5 g per 100 ml which corresponds to the fat content of human breast milk, which is in the range of 30-40 g/L.
Table 3 shows the fatty acid composition of Fat blend 11 comprising a fat base of the invention (30%) which is mixed/blended with other oils and fats used to create a fat source used in an infant formula for use in the invention. Table 4 shows details of the ingredients and properties of the infant formula comprising the fat source of Table 3. Since fat blends are prepared by blending fat base with other oils, the fatty acids composition of the blends results from the fatty acids composition of both the fat base and of the other oils mixed with the fat base.
TABLE 3
Fatty acid
% of fatty acids
C10:0
1.3
C12:0
10.3
C14:0
4.3
C16:0
23.5
C16:0 at sn-2 of total fatty acids
30.3
at sn-2
Ratio (%) of sn-2 palmitic acid
43
of total palmitic acid
C18:0
3.2
C18:1
39.2
C18:2
13.6
C18:3
1.7
C20:0
0.3
C20:1
0.3
C22:0
0.2
All numbers represent % (w/w), except the ratio which is defined as %.
C16:0 represents the total palmitic acid content.
C16:0 at the sn-2 represents the % palmitic acid at sn-2 of total sn-2 positioned fatty acids.
The ratio means the % of sn-2 palmitic acid of total palmitic acid {(% of sn-2 palmitic of total sn-2 positioned fatty acids)/3)/(% total palmitic acid)} × 100.
TABLE 4
Per 100 g
Per 100 ml
Formula
powder
ready to feed
Energy (kcal)
508
68
Sodium (mg)
140
18.8
Protein (g)
11.4
1.5
(Lacatalbumin/Casein 60/40)
Fat (gr)
26.5
3.5
Saturated fat (gr)
11.3
1.49
Linoleic acid (mg)
5000
670
Alpha-linolenic acid (mg)
530
71
Arachidonic acid (mg)
115
15.3
Docosahexaenoic acid (mg)
108
14.4
Cholesterol (mg)
2
0.3
Lactose (gr)
56
7.5
Calcium (mg)
430
57.3
Phosphorus (mg)
250
33.5
Potassium (mg)
420
56.3
Chloride (mg)
300
40.2
Iron (mg)
5.25
0.7
Magnesium (mg)
50
6.7
Zinc (mg)
3.5
0.47
Copper (mcg)
300
40.2
Manganese (mcg)
45
6
Iodine (mcg)
45
6
Taurine (mg)
45
6
Vitamin A I.U.
1500
200
Vitamin D I.U.
300
40.2
Vitamin E (mg)
10
1.3
Vitamin K (mcg)
45
6
Vitamin C (mg)
60
8
Vitamin B1 (mcg)
400
53
Vitamin B2 (mcg)
800
127
Vitamin B6 (mcg)
375
50
Vitamin B12 (mcg)
1.15
0.2
Niacin (mg)
6
0.8
Panthothenic acid (mg)
3
0.4
Folic acid (mcg)
67
9
Biotin (mcg)
14.3
1.9
Choline (mg)
37.5
5
Inositol (mg)
22.5
3
Moisture %
3
The level of fat and the exact composition can be controlled in order to yield infant formulas designed to mimic the different lactation periods.
Table 5 shows the fatty acid composition of Fat blend 12 comprising a fat base of the invention blended with other oils and fats used to create a fat source used in an infant formula for use in the invention.
TABLE 5
% from total Fatty acids
Fatty acid
C8:0
1.6
C10:0
1.5
C12:0
10.6
C14:0
3.9
C16:0
17.2
C16:0 at sn-2 of total fatty acids
26.3
at sn-2
Ratio (%) of sn-2 palmitic acid of
51
total palmitic acid
C18:0
2.4
C18:1
41.1
C18:2
18.2
C18:3
2.2
% fat base (concentrate) in fat
43
blend
Vegetable Oil
Randomized Coconut oil
22
Randomized Sunflower
15
Randomized Rapeseed
20
All numbers represent % (w/w), except the ratio which is defined as %.
C16:0 represents the total palmitic acid content.
C16:0 at the sn-2 represents the % palmitic acid at sn-2 of total sn-2 positioned fatty acids.
The ratio means the % of sn-2 palmitic acid of total palmitic acid {(% of sn-2 palmitic of total sn-2 positioned fatty acids)/3)/(% total palmitic acid)} × 100.
Effect of Fat Blend on Gastro-Intestinal (G) Tolerance and Intestinal Maturity
The effect of fat bases and fat blends of the present invention on GI tolerance and intestinal maturity is examined by a clinical study in animal models, in (i) prematurely born rats (Ito Y et al, Intestinal microcirculatory dysfunction during the development of experimental necrotizing enterocolitis Pediatric Research 2007), and (ii) in neonate rat model (Dvorak B, Epidermal growth factor reduces the development of necrotizing enterocolitis in a neonatal rat model, Am J Physiol Gastrointest Liver Physiol. 2002) which both represent models of preterm infants.
The study includes three groups of animals that receive formulas that differ only in their fat composition, mainly the palmitic acid content. One group is administered standard rat milk substitute (that mimics rat milk), the second group is administered rat milk substitute that contains a palmitic acid fat content of about 8% of total fatty acid, of which about 10% is at sn-2 position of the triglyceride and the third group is administered a rat milk substitute that contains fat blend 1 (see Table 2) which contains a total palmitic acid fat content of about 20% of fatty acid, of which ˜50% is at sn-2 position of the triglyceride. The formula is administered to all groups for 3 months and their GI tolerance is examined by detailed known GI tolerance and general health at baseline and during the study approximately every month. Further, the intestinal maturity of the study subjects is examined by histological assays at the end of the study. The animals in the first and third group demonstrate better GI tolerance and intestinal maturity than the second group as determined by statistical analysis of questionnaires and by the histological tests. The animals in the third group demonstrate even better GI tolerance and intestinal maturity than the first group as determined by statistical analysis of questionnaires and by the histological tests.
The efficacy of a fat blend (see Table 2) on enhancing intestinal growth, development and maturation was investigated in an animal model study. Animals fed with a diet enriched with a high content of palmitic acid at the sn-2 position (Fat blend 6) were compared to animals fed with parallel diets, which contained either similar concentration of palmitic acid or low concentration of palmitic acid.
Study Design
60 Male Sprague-Dawley rats were obtained from the Harlan Laboratories (Rehovot, Israel) at 21 days of age, immediately after weaning and at body weight of 40-50 g.
The rats were randomly assigned to receive one of 3 different diets (see Tables 6 and 7); the diets supplied were different only in their fat content:
Following the 8th or 15th day of feeding, animals were anesthetized, sacrificed and the small intestine was removed and divided into three segments: duodenum, proximal jejunum and terminal ileum. The small intestine segments were used for gross pathology, morphology and histological assays, which indicate intestinal maturity of the study animals.
Diets
All diets were identical with respect to nutrient content and differed only with respect to the type of oil (Tables 6 and 7).
TABLE 6
Fatty acids composition of supplemented oils (% of total fatty acids)
Fatty acid
Preparation
Preparation
(% from total FA)
Fat blend 6
control I
control II
C8
0.6
0.6
1
C10
0.7
0.6
0.9
C12
8.1
8.2
13.2
C14
2.9
3.3
4.6
C16
21.6
22.6
8.2
C16:0 at sn-2 of total
31.3
9.1
2.8
fatty acids at sn-2
Ratio (%) of sn-2
48.3
13.4
11.4
palmitic acid of total
palmitic acid
Palmitic acid at sn-2 of
66
37
11
total saturated fatty
acid at sn-2
C18
2.6
3.5
2.7
C18:1
42.7
41.9
47.3
C18:2
18
16.4
18.8
C18:3
1.8
1.7
1.9
others
0.90
4.6
1.4
All numbers represent % (w/w), except the ratio which is defined as %.
C16:0 represents the total palmitic acid content.
C16:0 at the sn-2 represents the % palmitic acid at sn-2 of total sn-2 positioned fatty acids.
The ratio means the % of sn-2 palmitic acid of total palmitic acid {(% of sn-2 palmitic of total sn-2 positioned fatty acids)/3)/(% total palmitic acid)} × 100.
Palmitic acid at sn-2 of total saturated fatty acid at sn-2 represents the % palmitic acid at sn-2 of total sn-2 positioned saturated fatty acids.
TABLE 7
Diet Compositions
Diet A
Diet B
Diet C
Protein (% by weight)
19.1
19.1
19.1
Carbohydrate (% by weight)
61.9
61.9
61.9
Fat (% by weight)
6.2
6.2
6.2
Calories (kcal/gr)
3.8
3.8
3.8
Fat blend 6 (g/kg)
60
Preparation control I (g/kg)
60
Preparation control II (g/kg)
60
Food Consumption
During the feeding period, body weight and non-consumed food were weighed twice weekly. Food intake was calculated and expressed as grams per day. Energy and fat intake were calculated corresponding to the amount of ingested food.
Intestinal Gross Pathology and Morphology Analysis
The small intestine was removed and divided into three segments: duodenum, proximal jejunum and terminal ileum. Each segment was weighed and the weight per cm of bowel length was calculated. The segments were opened; bowel circumference in every segment was measured in three different sites and mean bowel circumference was calculated. Mucosa was scraped off and weighed. Bowel and mucosal weight was expressed as mg/cm bowel length/100 g body weight.
Histological Changes Analysis
Histological sections were prepared from the jejunal and ileal remnants.
The intestine for histology was split on the antimesenteric border and washed with iced saline. Pieces of proximal jejunum immediately distal to Treitz ligament and terminal ileum near the ileo-cecal junction were fixed for 24 hours in 5% formalin, washed with absolute alcohol, and embedded in paraffin. Transverse 5 min sections were prepared in a standardized fashion and were stained with Hematoxylin and Eosin. The villus height and crypt depth was measured using the Image Pro Plus 4 image analysis software (Media Cybernetics, Baltimore, Md., USA) and expressed in μm.
Enterocyte Proliferation
Crypt cell proliferation was assessed using a biotinylated monoclonal anti-BrdU antibody system provided in a kit form (Zymed Laboratories, Inc, San Francisco, Calif.). Standard 5-bromodeoxyuridine (5-BrdU) labeling reagent (Cat. No. 00-0103, Zymed Laboratories, Inc, San Francisco, Calif.) was injected intraperitoneally at a concentration of 1 ml/100 g body weight 2 hours before sacrifice. Tissue slices (5 μm) were deparaffinized and rehydrated with xylene and graded alcohol. The slides were heated for 10 minutes in citrate buffer, pre-treated with denaturating solution for 20 minutes, and incubated with blocking solution for 10 minutes. The sections were stained with a biotinylated monoclonal anti-BrdU antibody for 60 minutes and were then treated with streptavidin-peroxidase for 10 minutes. BRDU-positive color development was obtained by incubating the sections with DUB mixture for 3-5 minutes. An index of proliferation was determined as the ratio of crypt cells staining positively for BrdU per 10 crypts (Shamir et al., 2005, Digestive Diseases and Sciences, Vol. 50, No. 7 pp. 1239-1244 and Sukhotnik et al., 2008 Dig Dis Sci.; Vol 53(5):1231-9).
Results
Energy Intake, Food and Fat Intake
Food intake increased significantly during the two week period in all animals, without a statistically significant difference between the experimental groups.
Intestinal Mucosal Parameters
Effects of dietary treatment on intestinal mucosal parameters were different in proximal and distal intestine. The tested intestinal mucosal parameters were bowel circumference, bowel weight and mucosal weight. Those parameters indicate the physiological development of the intestinal tissue.
In Proximal Intestine
In proximal intestine (jejunum and duodenum), following one week of feeding, rats from the diet A group demonstrated statistically significant higher bowel and mucosal weight compared to diet C group (Table 8). It should be emphasized that deprivation of palmitic acid in diet C resulted in initial signs of mucosal hypoplasia, which became more prominent after 2 weeks of the dietary treatment. After two weeks of feeding, rats from the diet A group demonstrated a trend towards an increase in bowel weight in jejunum when compared to diet B and diet C animals. Mucosal weight of animals fed with diet A was significantly higher compared to diet C animals (p=0.027) (
In Ileum
In ileum, following one week of feeding there were no differences in bowel and mucosal weight between Diet A and Diet B. However rats who received Diet A and Diet B demonstrated greater mucosal weight compared with Diet C animals (Table 8). After two weeks of feeding, diet A exerted a greater bowel and mucosal weight than diet C. Moreover Diet A rats showed higher ileal mucosal weight compared to diet B group (p=0.048) (Table 8).
TABLE 8
Effects of dietary treatment on intestinal mucosal parameters
Parameters
Diet A
Diet B
Diet C
P value
One week feeding
bowel circumference
(mm)
Duodenum
8.0 ± 0.2
8.0 ± 0.3
8.2 ± 0.1
Jejunum
7.3 ± 0.3
7.1 ± 0.2
7.3 ± 0.3
Ileum
6.9 ± 0.2
6.3 ± 0.4
6.1 ± 0.3
0.031 A vs C
bowel weight (mg/cm/
100 gr BW)
Duodenum
69.7 ± 3.7
63.2 ± 3.5
61 ± 3.4
0.051 A vs C
Jejunum
54.4 ± 3.6
49.1 ± 3.8
45.7 ± 2.4
0.034 A vs C
Ileum
30.7 ± 2.2
32.1 ± 2.4
28.7 ± 2.8
mucosal weight (mg/
cm/100 grBW)
Duodenum
34.7 ± 2.5
29 ± 1.7
26.7 ± 2.1
0.044 A vs B
0.014 A vs C
Jejunum
26.9 ± 3
24.2 ± 3.2
20.5 ± 1.8
0.045 A vs C
Ileum
13.1 ± 0.6
13.4 ± 1.6
10.2 ± 1.3
0.029 A vs C
0.044 B vs C
Two week feeding
bowel circumference
(mm)
Duodenum
8.0 ± 0.2
8.6 ± 0.1
8.3 ± 0.2
0.028 A vs B
Jejunum
8.1 ± 0.2
7.8 ± 0.2
7.4 ± 0.1
0.007 A vs C
Ileum
7.6 ± 0.2
8.0 ± 0.2
6.7 ± 0.4
0.051 B vs C
0.054 A vs B
bowel weight (mg/cm/
100 gr BW)
Duodenum
53.5 ± 1.9
47.8 ± 2.3
48.9 ± 2.4
0.038 A vs B
Jejunum
38.3 ± 2.2
35.9 ± 1.5
34.7 ± 1.2
Ileum
29.0 ± 1.9
26.7 ± 1.9
24.5 ± 1.3
0.037 A vs C
mucosal weight (mg/
cm/100 gr BW)
Duodenum
24.3 ± 1.9
18.6 ± 1.9
20.2 ± 2.5
0.026 A vs B
Jejunum
16.9 ± 1.9
13.6 ± 1.4
13.6 ± 0.7
0.063 A vs C
Ileum
12.3 ± 1.7
9.2 ± 0.9
8.2 ± 0.9
0.027 A vs C
0.048 A vs B
Microscopic Changes
After one week, feeding diet C resulted in significant shortening of ileal villi compared with the other groups (Table 9). Those effects were enhanced following two weeks of feeding; diet A resulted in significantly greater microscopic changes compared with diet B and diet C (
TABLE 9
Effects of dietary treatment on microscopic changes
Microscopic
changes
Diet A
Diet B
Diet C
P value
One week feeding
Villus height
(μm)
Jejunum
475.6 ± 27
514.6 ± 26
447 ± 27.4
0.048 B vs C
Ileum
336.9 ± 36
281 ± 11.4
250.1 ± 10
0.015 A vs C
0.041 B vs C
Crypth depth
(μm)
Jejunum
199.3 ± 9.7
219.7 ± 15
194.9 ± 10
Ileum
158.6 ± 12
173.2 ± 11
154.3 ± 11
Two week feeding
Villus height
(μm)
Jejunum
502 ± 20
446 ± 29
497 ± 34.5
0.028 A vs B
Ileum
298 ± 24
230 ± 13
231.8 ± 23
0.018 A vs B
0.033 A vs C
Crypth depth
(μm)
Jejunum
252 ± 10
197 ± 7
206 ± 9
0.0015 A vs B
0.0016 A vs C
Ileum
179 ± 14
144 ± 7
147 ± 10
0.024 A vs B
0.04 A vs C
Enterocyte Proliferation
In Jejunum,
Following one week of feeding animals with diet A resulted in a significant increase in cell proliferation when compared to feeding animals with diet B and C, and feeding animals with diet B increased cell proliferation when compared to feeding rats with diet C. Following two weeks of feeding only diet A rats showed a significantly greater proliferation index in jejunum when compared to diet C rats (P=0.036) (
In Ileum
Following one week of feeding: diet A group exerted a strong stimulation of enterocyte proliferation when compared to diet C group (Table 10).
Following two weeks of feeding, diet A group exerted a strong stimulation of enterocyte proliferation in ileum. Animals fed with diet A showed a significantly greater proliferation index in ileum when compare to diet B and diet C animals (P=6.0004, 0.0001 respectively) (
TABLE 10
Effect of dietary treatment on enterocyte proliferation
enterocyte
proliferation
(BrdU
Positive
Cells/10
crypts)
Diet A
Diet B
Diet C
P values
One week feeding
Jejunum
176 ± 3.6
167 ± 3.2
159 ± 2.4
0.042 A vs B
0.0011 A vs C
0.041 B vs C
Ileum
151.1 ± 5.7
140.3 ± 3.7
134.3 ± 4.8
0.02 A vs C
Two week feeding
Jejunum
171.4 ± 4.4
164.3 ± 4.3
162 ± 3.4
0.036 A vs C
Ileum
170.3 ± 4.5
148.5 ± 2.7
132 ± 3.8
0.0004 A vs B
0.0001 A vs C
0.0017 B vs C
Thus, treatment with Diet A resulted in enhanced intestinal development and maturation, detected after the first week of dietary treatment and became more significant after two weeks of treatment. A marked increase in villus height is considered an important index of increased absorptive surface area in this group of animals. Increase in crypt cells along with hypertrophy of the individual cells, which was demonstrated morphometrically, is characteristic of tissues undergoing increased cell proliferation and/or repair.
Deprivation of palmitic acid in diet C resulted in hypoplastic changes in jejunum and especially in ileum. These changes appeared after one week of dietary treatment and increased after 2 weeks of dietary treatment, and they emphasized the detrimental effect of deprivation of palmitic acid. In addition, decrease in enterocyte proliferation was shown in rats fed with low palmitic diet can be considered a major mechanism, responsible for decreasing intestinal cell mass and mucosal hypoplasia.
The dynamic process of intestinal cell turnover is a function of crypt cell proliferation rates, migration along the crypt-villus axis, enterocyte differentiation, and cell death via apoptosis. A significant increase in cell proliferation following Diet A administration was accompanied by a trend toward increase in cell apoptosis, suggesting accelerated cell turnover during intestinal growth.
In conclusion, a high amount of palmitic acid of which a high amount is conjugated at the sn-2 position is an important factor in intestinal growth in post-weaning rats. Diet A resulted in prominent enhanced intestinal development, growth and maturation compared with diets containing a mix of standard vegetable oil mixed with compositions with a high content of palmitic acid or low content of palmitic acid. The prominent enhanced intestinal development, growth and maturation appeared after 1 week and was enhanced after 2 weeks of dietary treatment. Diet A further exerted greater stimulating effects on enterocyte proliferation and turnover compared to the other diets.
The reduction of calcium soap formation is a highly recognized and known beneficial effect of both oils enriched with palmitic acid esterified at sn-2 position and oils with low palmitic acid content (Koo et al., 2006, Journal of American college of Nutrition, Vol 25, No 2 pp 117-122). This effect is similar between these oils and is known to attribute to reducing discomforts and symptoms related to food digestion.
Since Diet A (in the examples above) demonstrated superior and significantly different effects on intestinal development and maturation as compared to Diet C, it is evident that these effects of enhanced intestinal development and maturation are not related to, nor associated with the effect of reducing calcium soap formation.
The effect of a fat blend on proliferation and differentiation in tissue culture was examined in Caco-2 cells. The Caco-2 cell line has been used to date in many qualitative and quantitative studies as an in vitro intestinal epithelial cell model. The cells are grown on permeable inserts from tight-junctions and attain many of the morphological and functional characteristics of small intestinal enterocytes (Artursson P., Karlsson J., 1991, Biochem. Biophys. Res. Commun., Vol 175, 880-885). This cellular model system demonstrated the positive effect of a fat supplement of the invention on intestinal maturation, through cell proliferation and paracellular permeability.
Study Design
Caco-2 cells, originating from a human colorectal carcinoma, were provided by the ATCC (American Type Culture Collection, ATCC® Number HTB-37).
Cells were propagated in Caco-2 Growth Medium under sterile conditions. The cells were subcultured twice prior to treatment. The cell cultures were incubated at 37±1° C., 5±0.5% CO2 and 95±5% humidity, in plastic flasks (NUNC). Caco-2 cellular differentiation and maturation were assessed by cells confluence and paracellular transport
Confluence and Paracellular Transport
Confluence and paracellular transport were measured in Caco-2 cells seeded on polylester membrane inserts. Confluence and differentiation of the cell monolayer on membrane inserts were measured 7 and 9 days post seeding by the evaluation of the Trans-Epithelial-Electrical-Resistance (TEER) measurements. TEER measurements have become universally established as the most convenient, reliable and non-destructive method for evaluating and monitoring the growth of epithelial tissue cultures in vitro. The confluence of the cellular monolayer, which is a model for intestinal maturity, is determined by an increase in TEER. TEER was measured using the Millicell-ERS (Millipore) electrode during cell incubation in growth medium containing 2 μM of the tested items:
TABLE 11
Fatty acids composition of a supplemented oil and a fat blend (% of total
fatty acids) before final assay concentrations dilution
high palmitic
fatty acid (as % from
acid enriched at sn-
low palmitic acid
total Fatty acid)
2 content oil (Fat blend 7)
content oil
C8
0.6
1.1
C10
0.6
1.0
C12
8.7
14.05
C14
3.5
4.9
C16
21
8.3
C16:0 at sn-2 of total
31.8
2.9
fatty acids at sn-2
Ratio (%) of sn-2
50.5
11.9
palmitic acid of total
palmitic acid
C16:1
0.00
0.1
C18
2.6
2.6
C18:1
44.4
47.6
C18:2
16.4
18.1
C18:3
1.5
1.6
C20
0.2
0.3
C20:1
0.3
0.4
All numbers represent % (w/w), except the ratio which is defined as %.
C16:0 represents the total palmitic acid content.
C16:0 at the sn-2 represents the % palmitic acid at sn-2 of total sn-2 positioned fatty acids.
The ratio means the % of sn-2 palmitic acid of total palmitic acid {(% of sn-2 palmitic of total sn-2 positioned fatty acids)/3)/(% total palmitic acid)} × 100.
Results
Confluence Parameters
Seven days post seeding, the Caco-2 cell's TEER value in the presence of LPO oil, was 233±59 ohms/cm2. Following an additional two days i.e. 9 days post seeding the Caco-2 cell's TEER value increased by 119.4 (
Conclusion: the in vitro model showed that Fat blend 7 incubation does not interfere with Caco-2 cells proliferation and differentiation, contrary to incubation with an oil with a low content of palmitic acid. The results indicate that Fat blend 7 promotes intestinal development and faster maturity, while an oil with a low palmitic acid content interferes with intestinal development.
The effect of diets with different palmitic acid content on prevention and treatment of short bowel syndrome as well as improving intestinal maturation and adaptation is investigated in an animal model study.
Study Design
Animals after either a bowel transection with re-anastomosis or partly small bowel resection are randomly assigned to one of the diet groups that differ only in their palmitic acid content. Following a feeding period, animals are sacrificed and the histological parameters of intestine and the proliferation and apoptosis of enterocytes are studied.
The Study is Performed in Two Phases:
All diets are identical with respect to nutrient content and differ only in palmitic acid content:
Animals are anesthetized and operated; the abdomen is opened by midline incision. In animals that undergo a partly small bowel resection, a 75% resection is performed, preserving the vascular arcade and leaving 5 cm of proximal jejunum and 10 cm of distal ileum. Intestinal continuity is restored by an end-to-end single layer anastomosis. In animals that undergo bowel transection with re-anastomosis, the intestine is divided and re-anastomosed without resection. Following laparotomy, all animals have access to water for the first 24 h following operation (Sukhotnik et al., 2004, Pediatr Surg Int Vol 20 (4): 235-239).
Food Consumption
During the feeding period, before and after operation, body weight and non-consumed food are weighed. Food intake is calculated and expressed as grams per day. Energy and fat intake are calculated corresponding to the amount of ingested food.
The study demonstrates that early exposure of an animal to Diet I results in improving the recovery from short bowel syndrome. Further, exposure of animals after short bowel syndrome induction to Diet I results in increase in overall intestinal wall and mucosal weights and in better recovery rates from short bowel syndrome as shown by the improvement in mucosal adaptation following bowel resection/induction. Animals receiving Diet I have greater mucosal hyperplasia responses in the remaining gut and greater stimulating effects on intestinal re-growth compared to animals receiving other diets.
The effect of diets with different palmitic acid content on prevention and treatment of necrotizing enterocolitis (NEC) is investigated in a hypoxia-hypothermia-formula-fed preterm animal model study.
Study Design
Animals are randomly assigned to one of the diet groups that differ only in their palmitic acid content.
The Study is Performed in Two Phases:
Experimental NEC is developed by the following procedure; new born pups, starting from 2 hr of age and then every 12 hr, are challenged with hypoxia by breathing 100% nitrogen gas in a closed, clear plastic chamber for 60 see, followed by hypothermia, exposure to cold at 4° C. for 10 min.
Diets
All diets are identical with respect to nutrient content and differ only in palmitic acid content.
To study the incidence and severity of NEC, the first feeding with the tested diets starts at 24 hr of age. The pups are randomly assigned to one of diet groups that differ only in their palmitic acid content. The animals are fed from birth by orogastric gavage. All pups are observed hourly for clinical signs of NEC such as abdominal distension, respiratory distress, and lethargy. 96 hours after birth, or at signs of illness, the pups are euthanized via decapitation (Travadi et al., 2006, Pediatr Res. Vol 60(2): 185-9). Followed euthanized, the animal's intestinal tissue is processed and examined for gross and histological scoring of damage (NEC).
To study the effects of diets on intestine recovery, animals are fed with the different diets after NEC induction. Intestinal epithelial cell migration (restitution) and proliferation, that are key elements in recovery from intestinal injury, are studied.
To investigate the effect of different diets on enterocyte proliferation and migration, bromodeoxyuridine is administered intraperitoneally 18 hours before sacrifice, with intestine subjected to bromodeoxy-uridine immunohistochemistry (Feng J, Besner G E., 2007, J Pediatr Surg. Vol; 42(1):214-20).
The study demonstrates that early exposure of an animal to Diet I results in reducing the incidence and severity of NEC. Further, exposure of animals developing clinical signs of NEC illness to Diet I, results in prevention of overall intestinal integrity damage or loss of mucosa. Animals receiving Diet I demonstrate less profound pathologic changes of NEC compared to animals receiving other diets.
The ability of high palmitic acid at sn-2 position to protect the intestines from NEC is due, in part, to its ability to preserve enterocyte migration and proliferation.
The effect of diets with different palmitic acid content on prevention and treatment of inflammatory bowel diseases, such as Crohn's disease (CD) and ulcerative colitis (UC), is investigated in an animal model study.
Study Design
Animals developing inflammatory bowel diseases by administration of dextran sulfate sodium (DSS) in their drinking water are randomly assigned to one of diet groups that differ only in their palmitic acid content.
The Study is Performed in Two Phases:
AU diets are identical with respect to nutrient content and differ only in palmitic acid content.
Administration of DSS in the drinking water of rodents is widely used as an experimental model of UC because it results in acute and chronic colitis and shares clinical and histopathological characteristics with human UC. DSS is a sulfated polymer that induces patchy mucosal injury in a dose-dependent manner. It also induces inflammation, initially through a direct toxic effect on epithelial cells, thereby leading to the development of severe colitis (Vicario et al, 2007, J Nutr.; Vol 137(8): 1931-7).
Food Consumption
During the feeding period, body weight and non-consumed food are weighed. Food intake is calculated and expressed as grams per day. Energy and fat intake are calculated corresponding to the amount of ingested food.
Analyses
For the prevention study, animals are randomly assigned to the different diets. After a feeding period each group is randomly divided into two experimental groups, one receives DSS in their drinking water and the other receives only tap water and the incidence and severity of inflammatory bowel disease are monitored, by measuring of production of some of the mediators involved in the intestinal inflammatory response, such as leukotriene B(4) (LTB(4)), tumor necrosis factor alpha (TNFalpha) and nitric oxide (NO) (Camuesco D, 2005, J Nutr. Vol; 135(4):687-94).
For the treatment study, survivors of inflammatory bowel disease are randomly assigned into diet groups and fed with the different diets. Following a treatment period, animals are monitored for clinical findings (body weight loss, bloody diarrhea, reduced physical activity, severe anemia, shortened colonic length, and perianal injury) (Kishimoto S, 2000, Dig Dis Sci. Vol; 45(8):1608-16).
Animals are sacrificed and intestinal adaptation is evaluated by histopathological findings (pathological lesion score) and analysis of mucosal villus height (VII), crypt depth (CD), total mucosal height, bromodeoxyuridine (BrdU) incorporation, an index of cell proliferation, and full-thickness DNA and protein content as measures of intestinal adaptive growth (Evans M E, 2005, JPEN J Parenter Enteral Nutr. Vol ;29(5):315-20).
The study demonstrates that early exposure of animal to Diet I results in reducing the occurrence of inflammatory bowel diseases. Further, feeding of animals after inflammatory bowel diseases induction to Diet I results first, in decreasing events occurring in the colonic mucosa (breakdown of the epithelial mucosal barrier and higher infiltration of neutrophils) and further, in decrease of induction of severe colitis with diarrhea and colonic mucosal lesions. Total positive alteration in of mucosal function and the inflammation is indicated following feeding of the animals with Diet I.
The effect of diets with different palmitic acid content on energy absorption, caloric intake and fat malabsorption associated with short bowel syndrome are investigated in an animal model study.
Study Design
Animals after induction of short bowel syndrome by partly small bowel resection are randomly assigned to one of the diet groups that differ only in their palmitic acid content. Followed feeding, the effect of the different diets on fat malabsorption and intestinal uptake is monitored. It is commonly assumed that when the gastrointestinal symptoms are improved, the amount of energy available from the diet is improved.
Operation
Animals are anesthetized and operated; the abdomen is opened by midline incision. In animals that undergo a partly small bowel resection, a 75% resection is performed, preserving the vascular arcade and leaving 5 cm of proximal jejunum and 10 cm of distal ileum. Intestinal continuity is restored by an end-to-end single layer anastomosis. In animals that undergo bowel transection with re-anastomosis, the intestine is divided and re-anastomosed without resection. Following laparotomy, all animals have access to water for the first 24 h following operation (Sukhotnik et al., 2004, Pediatr Surg Int Vol 20 (4): 235-239).
Food Consumption
During the feeding period, before and after operation, body weight and non-consumed food are weighed. Food intake is calculated and expressed as grams per day.
Analyses
Stool energy losses and the sources of energy within the stool are determined.
Following dietary treatment, stool samples are collected, as are food records. Stools are analyzed for gross energy, total nitrogen, fat content, and fatty acid concentration. Total caloric excretion is tested. The energy content per gram of stool samples is measured by ballistic bomb calorimetry (Miller P S, Payne P R. 1959, A ballistic bomb calorimeter. Br. J. Nutr; Vol 13:501-8) on a sample of freeze dried stool. (Murphy et al., 1991, Archives of Disease in Childhood; Vol 66: 495-500).
Diets
All diets are identical with respect to nutrient content and differ only in palmitic acid content.
The study demonstrates that Diet I results in improving the continuing fat malabsorption and energy uptake and decrease stool energy extraction in short bowel syndrome.
Further, exposure of animals after short bowel syndrome induction to diet I results in better recovery rates from short bowel syndrome.
The effect of diets with different palmitic acid content on prevention of alterations in intestinal permeability associated with inflammatory bowel diseases, such as Crohn's disease (CD) and ulcerative colitis (UC), is investigated in an animal model study.
Study Design
Animals developing inflammatory bowel diseases by administration of dextran sulfate sodium (DSS) in their drinking water are randomly assigned to one of diet groups that differ only in their palmitic acid content. Dietary treatment is administered after administration of DSS and the effect of the different diets on intestinal permeability is studied using bacterial lipopolysaccharide (LPS) leakage from the intestine by examining blood levels of LPS after intestinal loading was applied.
Diets
All diets are identical with respect to nutrient content and differ only in palmitic acid content
Administration of DSS in the drinking water of rodents is widely used as an experimental model of UC because it results in acute and chronic colitis and shares clinical and histopathological characteristics with human UC. DSS is a sulfated polymer that induces patchy mucosal injury in a dose-dependent manner. It also induces inflammation, initially through a direct toxic effect on epithelial cells, thereby leading to the development of severe colitis (Vicario et al, 2007, J Nutr.; Vol 137(8): 1931-7).
Food Consumption
During the feeding period, body weight and non-consumed food are weighed. Food intake is calculated and expressed as grams per day. Energy and fat intake are calculated corresponding to the amount of ingested food.
Analyses
Survivors of inflammatory bowel disease are randomly assigned into diet groups and fed with the different diets. Following a treatment period, animals are monitored for clinical findings (body weight loss, bloody diarrhea, reduced physical activity, severe anemia, shortened colonic length, and perianal injury) (Kishimoto S, 2000, Dig Dis Sci. Vol; 45(8):1608-16) and intestinal permeability assay is preformed.
Intestinal Permeability Assay
To evaluate the effect of the different diets on intestinal permeability, bacterial lipopolysaccharide (LPS; Escherichia coli serotype 0111:B4; Sigma-Aldrich) leakage from the intestine by examining blood levels of LPS after intestinal loading is applied. LPS is given to the animals by gavage. Thirty minutes after loading with LPS, the animals are sacrificed, and blood is collected for analysis by endotoxin assay using the limulus ameobocyte lystate (LAL) kit (BioWhittaker, Walkersville, Md.) (Lambert et al., 2003, J Pharmacol Exp Ther. Vol 305(3):880-6).
Feeding animals after inflammatory bowel diseases induction with Diet I results in prevention of increased intestinal permeability. Diet I feeding is causing a decrease in the levels of plasma endotoxin compared with Diet II and Diet III. The results show that the intestine of animals fed with Diet I is capable of restoring decreases in barrier function during recovery from inflammatory bowel disease.
Dror, Gai Ben, Cohen, Tzafra, Lifshitz, Yael, Bar-Yosef, Fabiana
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